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Corresponding author: Paul Schedl, Lewis Thomas Labs, Washington Rd., Princeton University, Princeton, NJ 08544., pschedl{at}molbio.princeton.edu (E-mail)
Communicating editor: K. ANDERSON
 | ABSTRACT |
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 TOP ABSTRACT MATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Drosophila melanogaster males have one X chromosome, while females have two. To compensate for the resulting disparity in X-linked gene expression between the two sexes, most genes from the male X chromosome are hyperactivated by a special dosage compensation system. Dosage compensation is achieved by a complex of at least six proteins and two noncoding RNAs that specifically associate with the male X. A central question is how the X chromosome is recognized. According to a current model, complexes initially assemble at 
35 chromatin entry sites on the X and then spread bidirectionally along the chromosome where they occupy hundreds of sites. Here, we report that mutations in Trithorax-like (Trl) lead to the loss of a single chromatin entry site on the X, male lethality, and mislocalization of dosage compensation complexes.
DROSOPHILA melanogaster males have one X chromosome, while females have two. To compensate for this disparity in gene dose, there are mechanisms to ensure that X-linked genes are expressed at the same level in the two sexes. One of these mechanisms is the hyperactivation of genes on the male X chromosome by a special dosage compensation system (reviewed in 
While a good deal is known about the assembly and mechanism of action of the MSL dosage compensation complex, it is not fully understood how the complex is specifically targeted to the X chromosome. The current model is based on the observation that in the absence of msl3, mle, or mof, Msl1 and Msl2 associate with 35 special, high-affinity sites on the X chromosome (
With the exception of JIL-1 (
Another gene that appears to function in both dosage compensation and sex-nonspecific vital processes is Trithorax-like (Trl;
| MATERIALS AND METHODS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Genetic crosses and fly stocks:
All crosses were performed at 22° in an incubator. Flies were grown on standard media. Trl13C and Trl62 are independent P-element-induced alleles (
The male-to-female ratio of flies carrying adult-viable combinations of Trl alleles described above was determined by combining data from crosses in several genetic backgrounds (i.e., different balancers and different directions of the cross). For each combination of alleles the ratio was not significantly different between genetic backgrounds (data not shown).
To assess the effects of msl mutants on the viability of males with incomplete Trl function, the following cross was performed,
where msl denotes alleles of msl1, msl2, mle and their combination that were used as described in Fig 2A and Table 1. Trl- is either Trl62 (for crosses described in Fig 2A and the top of Table 1) or Trl13C for the cross described in the bottom of Table 1 (for the latter cross, TM3,Ser balancer chromosome was used).
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To ensure that any effects seen in the experiment outlined above were not due to differences in genetic background, the following control cross was performed:
The male:female ratio of w; +/+; Trl13C/Trl62 flies obtained in this cross was then compared to the ratios obtained in the experimental crosses. The control for the cross involving the triple msl mutant combination in the Trl13C homozygous background was
The male:female ratios were compared as shown in Fig 1C.
The following crossing scheme was implemented to test the effects of the H83M2 transgene on the Trl mutant phenotype,
where Trl- denotes Trl13C, Trl62, or Trl2.3. Since fertility of Trl13C homozygous males is limited, we used several parallel crosses involving two or three different recombinant isolates between Trl13C and the H83M2-61 or H83M2-87A line to obtain enough progeny to score. The results for each Trl genotype and H83M2 line were then pooled. These crosses produced Trl mutant siblings that differed only in whether or not they carried the H83M2 transgene, thus minimizing the effects of genetic background.
Western blots:
Extract from 2.5 third instar larvae was loaded on an 8% polyacrylamide gel (PAGE). Western blotting was performed as described in
Staining of polytene chromosomes:
Larvae were grown at 22° on standard media regularly supplemented with water and yeast. Sex of larvae was determined either by size of gonads or by crossing y+ males with y- females. Salivary glands were dissected in PBS with 1% Tween-20 (Sigma, St. Louis) and fixed for 2 min in a drop of solution containing 50% acetic acid, 3.7% formaldehyde, and 1% Tween-20. Chromosomes were spread and stored in PBS with 0.05% Tween-20 at 4°. Slides were blocked for 30 min in 5% BSA [for rabbit anti-Msl1 (
Chromatin entry sites were visualized using the anti-Msl1 antibody. Salivary glands from w; Trl13Cmsl3H83M2-6I/+ and w; Trl13Cmsl3H83M2-6I/Trl2.3msl3 larvae were used to assess the effect of Trl on the distribution of chromatin entry sites. The X chromosomes in both of these classes of larvae came from the same w1 stock. Images were collected using the Zeiss LSM 510 confocal microscope.
Statistical tests:
For comparison within crosses, such as those illustrated in Fig 2B, the 
2 test was used with Microsoft Excel. Two-tailed Fisher's exact test was used to compare male:female ratios between crosses (such as in Fig 2, a and c, and Table 1), computed using a web-based program available at http://www.matforsk.no/ola/fisher.htm. Confidence intervals in Fig 1A were computed using the normal approximation of the binomial distribution.
| RESULTS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Trl mutations interfere with MSL-dependent dosage compensation:
Trl13C is the weakest Trl allele. A little more than half of the homozygotes survive to the adult stage (
Since sex-specific lethality in flies is usually associated with upsets in X chromosome dosage compensation, one possible explanation for the male lethal effects of these two Trl mutant combinations is that the reduction in Trl activity somehow perturbs the functioning of the msl dosage compensation system. If this is the case, one would predict that the male lethal effects seen in these two Trl mutant combinations would be exacerbated by reducing the dose of the msl genes. In an otherwise wild-type background, mutations in msl1 and msl2 are not haplo-insufficient, and heterozygous mutant males show little or no reduction in viability (not shown). However, as indicated in Fig 1B and Table 1, a reduction in the dose of either msl1 or msl2 substantially enhances the male lethality of the Trl13C/Trl62 mutant combination. By contrast, these msl mutations have little, if any, effect on the viability of Trl13C/Trl62 females. Similarly, reducing the dose of msl1, msl2, and mle together substantially increases the male lethal effects of the Trl13C/Trl62 mutant combination (Table 1). Whereas the viability of Trl13C/Trl62 mutant females carrying (or not carrying) the three MSL-complex mutants is only twofold less than that of sibling females heterozygous for Trl, the viability of Trl13C/Trl62 males carrying the triple MSL-complex mutant combination is reduced >10-fold. Since four independent chromosomes carrying various combinations of msl mutants were used, the enhancement we observed is unlikely to be due to second-site mutations unrelated to the dosage compensation system, although the precise magnitude of the effect is probably influenced by the genetic background, as seen from the different male viability resulting from the introduction of two independent msl1 alleles (Table 1). Additional support for the idea that a reduction in Trl activity may compromise the dosage compensation system comes from the effects of mutations in the msl complex on Trl13C homozygous males. Normally, Trl13C homozygous males are as viable as their sibling females (Fig 1A); however, when the dose of msl1, msl2, and mle is simultaneously halved, the viability of the Trl13C homozygous males is significantly reduced compared to their sibling females (Fig 1C).
While single mutations in msl1 and msl2 exacerbated the male lethal effects of the Trl13C/Trl62 mutant combination, no effects were observed for a mutation in mle (Fig 1B). This is most likely due to the fact that the Mle protein is present in excess, while Msl1 and Msl2 are thought to be limiting components of the MSL complex in males (
If the male lethality of Trl mutations is enhanced by reducing the amount of the MSL complex, we reasoned that it might be possible to suppress lethality by increasing the amount of complex. For this purpose, we used a transgene that constitutively expresses the Msl2 protein under the control of the hsp83 promoter (referred to as H83M2 transgene;
Trl mutant males possess a functional MSL complex:
One explanation for these gene dose effects is that Trl is required for the expression of a limiting component(s) of the MSL complex. To test this hypothesis, we compared Msl1 and Msl2 protein levels in wild-type and Trl mutant males. As illustrated for Msl1 in Fig 2A, we found that Trl mutations did not detectably alter the levels of either Msl1 or Msl2 proteins.
It could be argued that Trl mutations lead to the production of defective MSL complexes either because the expression of some other, perhaps unknown component of the dosage compensation system is substantially reduced or because Trl is required for the assembly of functional complexes. If either of these scenarios were correct, then mutations in Trl would be expected to suppress the lethal effects of ectopically expressing Msl2 protein in females from the H83M2 transgene. Contrary to this prediction, we found that Trl mutations enhance rather than suppress the lethal effects of the H83M2 transgene.
Under the conditions of the experiment shown in Fig 2B (growth at 22°), females carrying a single copy of the H83M2 transgene that are either wild type or heterozygous for Trl13C are almost fully viable (see legend to Fig 2). In contrast, when they are homozygous for Trl13C, there is a marked reduction in viability. For the H83M2-87A transgene line, viability is reduced to <50% of the Trl13C females lacking the transgene, while it is <10% for the H83M2-6I line. Even more striking reductions in viability are evident in H83M2 females trans-heterozygous for Trl13C and for either Trl62 or Trl23. In both of these cases, Trl mutant females carrying the transgene are never observed. The effects on female viability are unlikely to be due to some nonspecific interaction of the transgene with Trl, since female lethality can be rescued by reducing the dose of msl1 by half or by eliminating the function of either msl1 or mle (data not shown). These findings argue that the level and at least the global activity of the MSL complexes is not likely to be compromised by loss of Trl function.
Increased number of MSL-complex-bound autosomal sites in Trl mutant males:
Another hypothesis is that Trl may be required for association of the MSL complex with a subset of the 200 sites on the male X chromosome. To explore this possibility, we first compared the distribution of GAGA (Trl) protein and MSL complexes on polytene chromosomes from wild-type males. Double labeling experiments revealed that only 6 of the 50 X chromosomal sites bound by GAGA also have MSL complexes (Fig 3A). We next compared the distribution of MSL complexes on polytene chromosomes from wild-type and Trl mutant males. For these experiments we used two different Trl mutant combinations. In the first combination, Trl62/Trl2.3, we attempted to reduce the level of functional GAGA factor as much as possible. The Trl62/Trl2.3 mutant combination is lethal and the animals die during the third instar larval stage. Since the distribution of the MSL complex might be altered nonspecifically in these dying animals, we also used a second Trl mutant combination, Trl13C/Trl2.3. Trl13C/Trl2.3 third instar larvae are viable and develop much like wild type.
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Side-by-side comparison of polytenes from the two Trl mutant combinations and wild-type larvae failed to reveal any obvious gaps or striking discontinuities in the distribution of MSL complexes on the mutant X chromosome even at the sites that contain GAGA protein (Fig 3B). While there are no regions of the X chromosome in the Trl mutants in which MSL complexes are entirely missing, our assay is not sufficiently quantitative to detect modest reductions (two- to fourfold) in the amount of MSL complexes associated with the X chromosome or even with specific regions of the X chromosome. That the loading of the MSL complexes onto the X chromosome is, in fact, perturbed in Trl mutant males is suggested by the finding that the number of autosomal sites bound by MSL complexes is increased. This is illustrated in Fig 4, a and b. In wild-type males the number of autosomal sites for the Msl1 protein is 7 ± 1 and for the Msl2 protein is 5 ± 1. In the strong Trl mutant combination, Trl62/Trl2.3, the number of autosomal sites for Msl1 is 15 ± 1 and for Msl2 is 11 ± 1. This increase in the number of autosomal sites does not seem to be due to some nonspecific lethal effects in this Trl mutant combination because a similar increase is evident in the Trl13C/Trl2.3 mutant combination (see Fig 4B). Additional evidence for abnormalities in the distribution of the MSL complexes comes from the presence of MSL complexes at a site in the 3C region of the X chromosome of Trl mutant males that is unoccupied in wild-type males (Fig 3B, arrows). Similar results were obtained when we compared the distribution of MSL complexes in wild-type and Trl- females that ectopically express Msl2 protein from the H83M2 transgene (Fig 4C). As found in Trl males, the number of autosomal sites is increased.
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The presence of ectopic MSL sites on the autosomes in Trl mutants raises the possibility that male lethality arises from the hyperactivation of nearby genes. However, this suggestion seems unlikely since Trl13C/Trl2.3 males rescued by the H83M2 transgene have, if anything, an even larger number of ectopic autosomal sites for Msl2 (15 ± 1) than do Trl13C/Trl2.3 males lacking the transgene (13 ± 1, Fig 4B).
One chromatin entry site is missing in Trl mutant males:
Although Trl- males displayed no striking irregularities in the distribution of MSL complexes on the X chromosome, the presence of complexes at ectopic sites on the autosomes and X chromosome suggests that the distribution is abnormal and that some regions of the X chromosome may not have wild-type levels of the complex. This could arise, for example, if there were a defect in the loading of MSL complexes at one or more chromatin entry sites on the X chromosome. To investigate this possibility, we first compared the X chromosome distribution of GAGA and MSL-complex entry sites (Fig 5). Entry sites can be visualized because they are bound by Msl1 and Msl2 proteins in mle, msl3, or mof mutant backgrounds (35 chromatin entry sites on the X chromosome correspond to the genes encoding roX1 (position 3F) and roX2 (position 10C) RNAs, while the identity of the remaining sites is unknown. Both roX1 and roX2 have several (GA)n/(CT)n motifs that should be recognized by the GAGA factor. Moreover, these motifs are thought to be important for entry site function and are in hypersensitive sites in chromatin from male flies (33 entry sites, GAGA protein and the Msl complex appeared to colocalize only at one site, which is at 12DE. In unstretched chromosomes, GAGA protein and the MSL entry site at 12DE overlap; however, in favorable preparations (see Fig 5A) the GAGA band resolves into a tight "doublet" with the MSL complex in between.
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We next examined the association of the MSL complex with X chromosome entry sites in Trl mutants. We analyzed four chromosomes from four different slides for each genotype. The w1; msl3 83M2-6I Trl13C/msl3 Trl2.3 female larvae that looked healthy and were of a comparable developmental stage to the w1; msl3 83M2-6I/msl3 Trl2.3 control females were used. We were able to find a significant number of larvae to perform polytene squashes, presumably because mutations in msl3 rescue the effects of Msl2 expression in females. We found that the binding of MSL complexes to X chromosome entry sites in Trl- was identical to that in wild type except for the entry site at 12DE, the one that is flanked by GAGA protein. As illustrated in Fig 5B, the 12DE entry site is consistently absent in Trl- polytene chromosomes. This effect is not due to a polymorphism at this site, since the strains were isogenic for their X chromosomes (see MATERIALS AND METHODS).
| DISCUSSION |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Balancing gene expression from the sex chromosomes and autosomes is a critical process in organisms with sex differences in the number of sex chromosomes. In the fruit fly D. melanogaster, one of the mechanisms used to equalize expression levels in the two sexes is the hyperactivation of X-linked genes in male animals. The male dosage compensation system upregulates transcription by modifying the chromatin structure of X-linked genes. This is accomplished by a special multi-component complex that preferentially localizes to the X chromosome. Complex assembly depends most critically upon Msl1 and Msl2 and these two MSL proteins may provide some type of scaffold for recruiting/stabilizing other components of the complex. These other components include the two noncoding RNAs, roX1 and roX2, which have been implicated in targeting the complex to entry sites on the X chromosome. In addition, the chromatin-modifying enzymes themselves, Mof-1, a histone acetylase, and JIL-1, a tandem histone kinase, the putative helicase, Mle, and the Msl3 protein, are believed to associate with the complex through specific interactions. All but one of these factors appears to function primarily, if not exclusively, in the MSL dosage compensation system. The exception is the JIL-1 kinase that is required not only for proper dosage compensation, but also for other aspects of transcriptional regulation that are vital to both sexes. It would be reasonable to anticipate that other factors like JIL-1 that have crucial activities in dosage compensation while at the same time functioning in other processes that are important for both sexes will be identified. This seems to be true for the GAGA factor that is encoded by the Trl gene.
The importance of the GAGA factor in many aspects of gene regulation and chromatin dynamics has been extensively documented in previous studies (
Although Trl appears to function primarily in chromatin remodeling rather than as a dedicated component of the transcriptional machinery, it is involved in the expression of a very large and diverse array of genes. Since males must upregulate transcription of X-linked genes to achieve the same level of expression as females, it would be reasonable to suppose that males are likely to be much more dependent upon the proper functioning of the general transcriptional machinery than are females. Accordingly, any reduction in the activity of a factor critical for transcription would be expected to have considerably more deleterious effects on males than on females. If this idea is correct, then the male-specific lethality of Trl mutations could simply be due to a decline in the overall activity or efficiency of the transcriptional machinery rather than to an effect specific to the process of dosage compensation itself. This "impaired transcription" model would also explain why the male-specific lethal effects of Trl mutations are enhanced by a reduction in the dose of the msl genes and suppressed by increasing the dose of Msl2. Of course, this model predicts that hypomorphic mutations in components of the transcriptional apparatus should also exhibit male-specific lethality like mutations in Trl. Although some alleles of TAF250 do cause preferential male lethality (D. WASSARMAN, personal communication), there is no evidence that compromising the activity of other general transcription factors affects males more than females. In fact, none of the many hypomorphic mutations in the gene coding for the 140-kD subunit of RNA polymerase II give rise to male lethality (
An alternative, and we believe more plausible, explanation for the effects of Trl mutations on male viability is that the GAGA factor plays some important role in the functioning or activity of the msl-dependent dosage compensation system. In addition to accounting for both the male-specific lethality of Trl mutations and the genetic interactions between Trl and msl-complex genes, this suggestion would help explain two other findings. First, we observed abnormalities in the distribution of the MSL complexes in polytene chromosomes from Trl mutant males. These abnormalities include the presence of at least one ectopic site on the X chromosome and an increase in the number of autosomal sites. This redistribution of MSL complexes argues that the GAGA factor is important for correctly targeting the dosage compensation machinery to the X chromosome. A similar although more dramatic MSL redistribution was observed by 35 chromatin entry sites on the X chromosome, at 12DE, is missing in Trl mutants. Unlike any of the other chromatin entry sites observed in polytene chromosomes, GAGA is localized to the 12DE site. This finding argues that the GAGA factor is important in the formation/maintenance of this particular chromatin entry site. Neither of these effects on the chromosomal association of MSL complexes would be explained by a model in which the male-specific lethality of Trl mutations is due to some general reduction in the activity of the transcriptional machinery.
While it would be reasonable to propose that there is a direct connection between the defects in the chromosomal association of Msl complexes and male lethality, the precise mechanism is not entirely clear. One possibility is that male lethality is due to the loss of the 12DE entry site. Supporting this idea,
Although we believe that the loss of the 12DE entry could significantly impair the upregulation of genes in the 12C–F interval, there are at least two potential complications with this simple model. First, it seems unlikely that a reduction in the level of expression of genes in the 12C–F interval would in itself be sufficient to cause male lethality. Unless this chromosomal interval contains genes specifically required for male viability (e.g., encoding components of the dosage compensation machinery), this model would predict that this same interval is haplo-insufficient in females. However, there is no indication that deletions in this chromosomal interval have significant effects on female viability. Second, while the 12DE entry site is absent (in Trl; msl3 mutants), we do not see any obvious perturbation in the distribution of MSL complexes in this region of the X chromosome in Trl mutants that are wild type for the MSL genes. One explanation for this discrepancy is that defects in MSL-complex distribution in the vicinity of the 12DE site are obscured because the recruitment and spreading of complexes is much more robust in polytene chromosomes (which consist of hundreds of chromosomes whose sequences are aligned in precise register) than in chromosomes from polyploid or diploid nuclei. In fact,
This simple model would also not explain why MSL complexes in polytenes of Trl mutants localize to many ectopic sites on the autosomes. The presence of these autosomal complexes indicates that there must be some defect in the loading of complexes onto the X chromosome. Since we do not see any obvious reduction in the amount of complex in the 12C–F interval, it seems unlikely that the loss of the 12DE entry site alone could account for the presence of the autosomal complexes. Instead, this would suggest that the GAGA factor may be important in the loading or spreading of complexes from a number of entry sites located elsewhere on the X in addition to the 12DE entry site. In this respect, it is notable that the GAGA factor binds in close proximity to five MSL-complex entry sites, including roX1. If GAGA is important in the loading or spreading of complexes from a number of "Trl-dependent" entry sites in addition to 12DE, the male lethal effects of the Trl would be explained by the cumulative effects of a reduction in the expression of genes located in several different chromosomal regions rather than in just the 12C–F interval.
If loss of GAGA binding reduces the activity of only a subset of the chromatin entry sites, we would expect that dosage compensation would be compromised over some parts of the X chromosome, but not others. This would help to explain why the weak female lethal effects of the H83M2 transgene at 22° are greatly enhanced in Trl mutants. Under conditions in which Msl2 protein expression is limiting, defects in the spreading of MSL complexes from Trl-dependent entry sites could lead to a more efficient loading and subsequent spreading from sites that are independent of Trl function. Female lethality would be induced because of the increased concentration of complexes in regions served by "Trl-independent" entry sites. A hint that this may happen comes from the study of
Finally, it is important to note that the effects on MSL-complex distribution seen in salivary gland polytene chromosomes are unlikely to reproduce the defects in nonpolytene tissues that most directly contribute to male lethality. First, the available evidence suggests that GAGA interacts with different sites in different tissues (
An important question is how the GAGA factor functions in the formation and/or maintenance of the 12DE entry site. Given its role in generating nucleosome-free regions of chromatin, a plausible idea is that GAGA is required to ensure that the 12DE site is readily accessible to appropriate components of the MSL complex. In Trl mutants, the 12DE entry site and/or the immediately surrounding DNA would be packaged into a nucleosomal structure that cannot be used to initiate MSL-complex assembly, is refractory to the assembly of stable complexes, or is not compatible with the spreading of the complex in cis. The idea that a nucleosome-free region of chromatin is critical for entry site function is supported by recent studies of 200-bp sequence within the roX1 genes can direct the assembly of MSL complexes at ectopic sites and that this sequence is hypersensitive to nuclease digestion in male but not female chromatin. Further correlating the formation of a nuclease hypersensitive site with the assembly of MSL complexes,
In light of the effects of Trl mutations on male viability, it is interesting to note that the internal nuclease hypersensitive site in the roX1 and roX2 genes harbors potential GAGA-factor-binding sites. Moreover, these potential GAGA-binding sites appear to be important for the entry site function of these elements (
| FOOTNOTES |
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1 Present address: Department of Ecology and Evolution, University of Chicago, Chicago, IL 60637. 
2 Present address: Department of Embryology, Carnegie Institution of Washington, Baltimore, MD 21210.
| ACKNOWLEDGMENTS |
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We thank R. Kelley and M. Kuroda for providing fly stocks and antibodies generously and promptly. The GAGA-581 antibody was a gift of C. Benyajati. M. A. Mortin, S. M. Parkhurst, D. Ish-Horowitz, M. Mlodzik, and D. Wassarman provided crucial unpublished information. We are grateful to G. Deshpande and J. Huie for critical reading of the manuscript. This work was supported by a National Institutes of Health (NIH) grant to P.S. and NIH training grants to A.J.G. and J.L.Y.
Manuscript received March 13, 2003; Accepted for publication October 6, 2003.
| LITERATURE CITED |
|---|
| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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BAKER, B. S., M. GORMAN, and I. MARIN, 1994 Dosage compensation in Drosophila.. Annu. Rev. Genet. 28:491-521.[CrossRef][Medline]
BASHAW, G. J. and B. S. BAKER, 1997 The regulation of the Drosophila msl-2 gene reveals a function for Sex-lethal in translational control. Cell 89:789-798.[CrossRef][Medline]
BENYAJATI, C., L. MUELLER, N. XU, M. PAPPANO, and J. GAO et al., 1997 Multiple isoforms of GAGA factor, a critical component of chromatin structure. Nucleic Acids Res. 25:3345-3353.
BHAT, K. M., G. FARKAS, F. KARCH, H. GYURKOVICS, and J. GAUSZ et al., 1996 The GAGA factor is required in the early Drosophila embryo not only for transcriptional regulation but also for nuclear division. Development 122:1113-1124.[Abstract]
BIGGIN, M. D. and R. TJIAN, 1988 Transcription factors that activate the Ultrabithorax promoter in developmentally staged extracts. Cell 53:699-711.[CrossRef][Medline]
BONE, J. R., J. LAVENDER, R. RICHMAN, M. J. PALMER, and B. M. TURNER et al., 1994 Acetylated histone H4 on the male X chromosome is associated with dosage compensation in Drosophila.. Genes Dev. 8:96-104.
CHANG, K. A. and M. I. KURODA, 1998 Modulation of MSL1 abundance in female Drosophila contributes to the sex specificity of dosage compensation. Genetics 150:699-709.
CLINE, T. W. and B. J. MEYER, 1996 Vive la difference: males vs females in flies vs worms. Annu. Rev. Genet. 30:637-702.[CrossRef][Medline]
CROSTON, G. E., L. A. KERRIGAN, L. M. LIRA, D. R. MARSHAK, and J. T. KADONAGA, 1991 Sequence-specific antirepression of histone H1-mediated inhibition of basal RNA polymerase II transcription. Science 251:643-649.
DESHPANDE, G., J. STUKEY, and P. SCHEDL, 1995 scute (sis-b) function in Drosophila sex determination. Mol. Cell. Biol. 15:4430-4440.[Abstract]
DESHPANDE, G., M. E. SAMUELS, and P. D. SCHEDL, 1996 Sex-lethal interacts with splicing factors in vitro and in vivo.. Mol. Cell. Biol. 16:5036-5047.[Abstract]
FARKAS, G., J. GAUSZ, M. GALLONI, G. REUTER, and H. GYURKOVICS et al., 1994 The Trithorax-like gene encodes the Drosophila GAGA factor. Nature 371:806-808.[CrossRef][Medline]
FRANKE, A. and B. S. BAKER, 1999 The roX1 and roX2 RNAs are essential components of the compensasome, which mediates dosage compensation in Drosophila.. Mol. Cell 4:117-122.[CrossRef][Medline]
GORMAN, M., A. FRANKE, and B. S. BAKER, 1995 Molecular characterization of the male-specific lethal-3 gene and investigations of the regulation of dosage compensation in Drosophila.. Development 121:463-475.[Abstract]
GRANOK, H., B. A. LEIBOVITCH, C. D. SHAFFER, and S. C. ELGIN, 1995 Chromatin. Ga-ga over GAGA factor. Curr. Biol. 5:238-241.[CrossRef][Medline]
GREENBERG, A. J. and P. SCHEDL, 2001 GAGA factor isoforms have distinct but overlapping functions in vivo.. Mol. Cell. Biol. 21:8565-8574.
GU, W., P. SZAUTER, and J. C. LUCCHESI, 1998 Targeting of MOF, a putative histone acetyl transferase, to the X chromosome of Drosophila melanogaster.. Dev. Genet. 22:56-64.[CrossRef][Medline]
HENRY, R. A., B. TEWS, X. LI, and M. J. SCOTT, 2001 Recruitment of the male-specific lethal (MSL) dosage compensation complex to an autosomally integrated roX chromatin entry site correlates with an increased expression of an adjacent reporter gene in male Drosophila.. J. Biol. Chem. 276:31953-31958.
HILFIKER, A., D. HILFIKER-KLEINER, A. PANNUTI, and J. C. LUCCHESI, 1997 mof, a putative acetyl transferase gene related to the Tip60 and MOZ human genes and to the SAS genes of yeast, is required for dosage compensation in Drosophila.. EMBO J. 16:2054-2060.[CrossRef][Medline]
JIN, Y., Y. WANG, D. L. WALKER, H. DONG, and C. CONLEY et al., 1999 JIL-1: a novel chromosomal tandem kinase implicated in transcriptional regulation in Drosophila.. Mol. Cell 4:129-135.[CrossRef][Medline]
JIN, Y., Y. WANG, J. JOHANSEN, and K. M. JOHANSEN, 2000 JIL-1, a chromosomal kinase implicated in regulation of chromatin structure, associates with the male specific lethal (MSL) dosage compensation complex. J. Cell Biol. 149:1005-1010.
KAGEYAMA, Y., G. MENGUS, G. GILFILLAN, H. G. KENNEDY, and C. STUCKENHOLZ et al., 2001 Association and spreading of the Drosophila dosage compensation complex from a discrete roX1 chromatin entry site. EMBO J. 20:2236-2245.[CrossRef][Medline]
KELLEY, R. L. and M. I. KURODA, 2000 The role of chromosomal RNAs in marking the X for dosage compensation. Curr. Opin. Genet. Dev. 10:555-561.[CrossRef][Medline]
KELLEY, R. L., I. SOLOVYEVA, L. M. LYMAN, R. RICHMAN, and V. SOLOVYEV et al., 1995 Expression of msl-2 causes assembly of dosage compensation regulators on the X chromosomes and female lethality in Drosophila.. Cell 81:867-877.[CrossRef][Medline]
KELLEY, R. L., J. WANG, L. BELL, and M. I. KURODA, 1997 Sex lethal controls dosage compensation in Drosophila by a non-splicing mechanism. Nature 387:195-199.[CrossRef][Medline]
KELLEY, R. L., V. H. MELLER, P. R. GORDADZE, G. ROMAN, and R. L. DAVIS et al., 1999 Epigenetic spreading of the Drosophila dosage compensation complex from roX RNA genes into flanking chromatin. Cell 98:513-522.[CrossRef][Medline]
KERRIGAN, L. A., G. E. CROSTON, L. M. LIRA, and J. T. KADONAGA, 1991 Sequence-specific transcriptional antirepression of the Drosophila Kruppel gene by the GAGA factor. J. Biol. Chem. 266:574-582.
LU, Q., L. L. WALLRATH, H. GRANOK, and S. C. ELGIN, 1993 CT)n (GA)n repeats and heat shock elements have distinct roles in chromatin structure and transcriptional activation of the Drosophila hsp26 gene. Mol. Cell. Biol. 13:2802-2814.
LUCCHESI, J. C. and J. E. MANNING, 1987 Gene dosage compensation in Drosophila melanogaster.. Adv. Genet. 24:371-429.[Medline]
LYMAN, L. M., K. COPPS, L. RASTELLI, R. L. KELLEY, and M. I. KURODA, 1997 Drosophila male-specific lethal-2 protein: structure/function analysis and dependence on MSL-1 for chromosome association. Genetics 147:1743-1753.[Abstract]
MELLER, V. H. and B. P. RATTNER, 2002 The roX genes encode redundant male-specific lethal transcripts required for targeting of the MSL complex. EMBO J. 21:1084-1091.[CrossRef][Medline]
MELLER, V. H., P. R. GORDADZE, Y. PARK, X. CHU, and C. STUCKENHOLZ et al., 2000 Ordered assembly of roX RNAs into MSL complexes on the dosage-compensated X chromosome in Drosophila.. Curr. Biol. 10:136-143.[CrossRef][Medline]
OH, H., Y. PARK, and M. I. KURODA, 2003 Local spreading of MSL complexes from roX genes on the Drosophila X chromosome. Genes Dev. 17:1334-1339.
PALMER, M. J., V. A. MERGNER, R. RICHMAN, J. E. MANNING, and M. I. KURODA et al., 1993 The male-specific lethal-one (msl-1) gene of Drosophila melanogaster encodes a novel protein that associates with the X chromosome in males. Genetics 134:545-557.[Abstract]
PALMER, M. J., R. RICHMAN, L. RICHTER, and M. I. KURODA, 1994 Sex-specific regulation of the male-specific lethal-1 dosage compensation gene in Drosophila.. Genes Dev. 8:698-706.
PANNUTI, A. and J. C. LUCCHESI, 2000 Recycling to remodel: evolution of dosage-compensation complexes. Curr. Opin. Genet. Dev. 10:644-650.[CrossRef][Medline]
PARK, Y., G. MENGUS, X. BAI, Y. KAGEYAMA, and V. H. MELLER et al., 2003 Sequence-specific targeting of Drosophila roX genes by the MSL dosage compensation complex. Mol. Cell 11:977-986.[CrossRef][Medline]
PARKHURST, S. M. and D. ISH-HOROWICZ, 1991 wimp, a dominant maternal-effect mutation, reduces transcription of a specific subset of segmentation genes in Drosophila.. Genes Dev. 5:341-357.
RAFF, J. W., R. KELLUM, and B. ALBERTS, 1994 The Drosophila GAGA transcription factor is associated with specific regions of heterochromatin throughout the cell cycle. EMBO J. 13:5977-5983.[Medline]
TSUKIYAMA, T., P. B. BECKER, and C. WU, 1994 ATP-dependent nucleosome disruption at a heat-shock promoter mediated by binding of GAGA transcription factor. Nature 367:525-532.[CrossRef][Medline]
WANG, Y., W. ZHANG, Y. JIN, J. JOHANSEN, and K. M. JOHANSEN, 2001 The JIL-1 tandem kinase mediates histone H3 phosphorylation and is required for maintenance of chromatin structure in Drosophila.. Cell 105:433-443.[CrossRef][Medline]
WILKINS, R. C. and J. T. LIS, 1997 Dynamics of potentiation and activation: GAGA factor and its role in heat shock gene regulation. Nucleic Acids Res. 25:3963-3968.
ZEIDLER, M. P., K. YOKOMORI, R. TJIAN, and M. MLODZIK, 1996 Drosophila TFIIA-S is up-regulated and required during Ras-mediated photoreceptor determination. Genes Dev. 10:50-59.
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